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芽孢杆菌属GL1黄原胶裂解酶的晶体结构,该酶作用于黄原胶的侧链。

Crystal structure of Bacillus sp. GL1 xanthan lyase, which acts on the side chains of xanthan.

作者信息

Hashimoto Wataru, Nankai Hirokazu, Mikami Bunzo, Murata Kousaku

机构信息

Department of Basic and Applied Molecular Biotechnology, Division of Food and Biological Science, Graduate School of Agriculture, Kyoto, Uji, Kyoto 611-0011, Japan.

出版信息

J Biol Chem. 2003 Feb 28;278(9):7663-73. doi: 10.1074/jbc.M208100200. Epub 2002 Dec 9.

DOI:10.1074/jbc.M208100200
PMID:12475987
Abstract

Xanthan lyase, a member of polysaccharide lyase family 8, is a key enzyme for complete depolymerization of a bacterial heteropolysaccharide, xanthan, in Bacillus sp. GL1. The enzyme acts exolytically on the side chains of the polysaccharide. The x-ray crystallographic structure of xanthan lyase was determined by the multiple isomorphous replacement method. The crystal structures of xanthan lyase and its complex with the product (pyruvylated mannose) were refined at 2.3 and 2.4 A resolution with final R-factors of 17.5 and 16.9%, respectively. The refined structure of the product-free enzyme comprises 752 amino acid residues, 248 water molecules, and one calcium ion. The enzyme consists of N-terminal alpha-helical and C-terminal beta-sheet domains, which constitute incomplete alpha(5)/alpha(5)-barrel and anti-parallel beta-sheet structures, respectively. A deep cleft is located in the N-terminal alpha-helical domain facing the interface between the two domains. Although the overall structure of the enzyme is basically the same as that of the family 8 lyases for hyaluronate and chondroitin AC, significant differences were observed in the loop structure over the cleft. The crystal structure of the xanthan lyase complexed with pyruvylated mannose indicates that the sugar-binding site is located in the deep cleft, where aromatic and positively charged amino acid residues are involved in the binding. The Arg(313) and Tyr(315) residues in the loop from the N-terminal domain and the Arg(612) residue in the loop from the C-terminal domain directly bind to the pyruvate moiety of the product through the formation of hydrogen bonds, thus determining the substrate specificity of the enzyme.

摘要

黄原胶裂解酶是多糖裂解酶家族8的成员,是芽孢杆菌属GL1中细菌杂多糖黄原胶完全解聚的关键酶。该酶对多糖的侧链进行外切作用。黄原胶裂解酶的X射线晶体结构通过多重同晶置换法测定。黄原胶裂解酶及其与产物(丙酮酸化甘露糖)复合物的晶体结构分别在2.3 Å和2.4 Å分辨率下进行了精修,最终R因子分别为17.5%和16.9%。无产物酶的精修结构包含752个氨基酸残基、248个水分子和一个钙离子。该酶由N端α螺旋结构域和C端β折叠结构域组成,分别构成不完全的α(5)/α(5)桶状结构和反平行β折叠结构。一个深裂隙位于N端α螺旋结构域中,面向两个结构域之间的界面。尽管该酶的整体结构与用于透明质酸和软骨素AC的8家族裂解酶基本相同,但在裂隙上方的环结构中观察到了显著差异。与丙酮酸化甘露糖复合的黄原胶裂解酶的晶体结构表明,糖结合位点位于深裂隙中,其中芳香族和带正电荷的氨基酸残基参与结合。来自N端结构域的环中的Arg(313)和Tyr(315)残基以及来自C端结构域的环中的Arg(612)残基通过形成氢键直接与产物的丙酮酸部分结合,从而决定了该酶的底物特异性。

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